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ViPR

This is a collection of scripts used for the analysis of RNA viruses, based on LoFreq. The main wrapper is vipr.py ("Viper" written in Python though :) which will create a makefile defining the pipeline setps and will subsequently call make. Some of these scripts are quite specific to small genomes, others you might able to reuse some of them for larger - e.g. bacterial - genomes.

WARNING: Use at your own risk: this pipeline is not based on a proper pipeline framework (but is being ported to ruffus at the moment), uses some outdated scripts, has a huge dependency list and might make assumptions that are not met in your setup.

Installation

The impatient can simply use the full path for calling the scripts in ./src or add that directory to their PATH variable.

For a proper installation, cd into this directory and then use

$ python setup.py

install --prefix for installing the scripts.

For more options see

$ python setup.py install -h

Note: if you're using a special prefix for installation, please make sure that the corresponding bin directory is in your PATH and the corresponding python library path is in your PYTHONPATH.

Dependencies

A (very likely) incomplete list of dependencies:

  • make
  • FastQC
  • Picard
  • GATK
  • Samtools
  • Python 2.7
  • BWA
  • Mummer (nucmer)
  • LoFreq > 0.5
  • pysam

Some scripts will complain if the dependencies cannot be found in standard paths, but they should all allow you to point them to the correct place with environment variables.

Usage

ViPR is basically just the (Makefile based) glue for running a series of scripts and external programs. The wrapper script is vipr.py

See

$ vipr.py -h

for help.

Mandatory options are:

  • -r reference: mapping reference fasta file
  • -1 reads: first fastq[.gz] file (use -2 in addition for paired end sequencing)
  • -p PRIMER_FA: a list of primers you used for amplification
  • -o OUT_DIR: the output directory in which output files will be stored

Output

vipr.py produces a lot of files from coverage plots, to consensus sequences and primer positions, as well as SNV predictions etc in the specified output directory. The output directory will contain a README.txt file that lists the important files. In brief, these are

  • recal.bam: quality recalibrated mapping file with PCR duplicates removed
  • mapping-success.txt: simple mapping success stats
  • coverage.pdf: coverage plot
  • cons_masked.fa: consensus/master sequence with primer regions masked
  • final.snp: filtered, low-frequency SNV predictions

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